Considerations for point-of-care diagnostics: evaluation of acridine orange staining and postprocessing methods for a three-part leukocyte differential test

Powless, Amy J.; Conley, Roxanna J.; Freeman, K.A.; Muldoon, Timothy J.

doi:10.1117/1.jbo.22.3.035001

Cited by 17 publications

(20 citation statements)

References 34 publications

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“…Users were not supplied with a timer or stopwatch and relied on their own judgment of the 3.5-minute incubation time of the blood with AO. While the fluctuation of the cell population fluorescence intensities within the 4-minute experiment time does not adversely affect our analysis, we speculate that when the incubation time becomes long, the granulocyte and monocyte populations become more challenging to distinguish, similarly to results recently reported by Powless et al [44] Further standardization of the incubation time through a more detailed protocol may eliminate even this minor effect.…”

Section: Comparison Between Results By Trained and Untrained Userssupporting

confidence: 79%

Performance of a cost‐effective and automated blood counting system for resource‐limited settings operated by trained and untrained users

Xie

Liu

Tong

et al. 2017

Journal of Biophotonics

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Current flow-based blood counting devices require expensive and centralized medical infrastructure and are not appropriate for field use. In this article we report a streamlined, easy-to-use method to count red blood cells (RBC), white blood cells (WBC), platelets (PLT) and 3-part WBC differential through a cost-effective and automated image-based blood counting system. The approach consists of using a compact, custom-built microscope with large field-of-view to record bright-field and fluorescence images of samples that are diluted with a single, stable reagent mixture and counted using automatic algorithms. Sample collection utilizes volume-controlled capillary tubes, which are then dropped into a premixed, shelf-stable solution to stain and dilute in a single step. Sample measurement and analysis are fully automated, requiring no input from the user. Cost of the system is minimized through the use of custom-designed motorized components. We compare the performance of our system, as operated by trained and untrained users, to the clinical gold standard on 120 adult blood samples, demonstrating agreement within Clinical Laboratory Improvement Amendments guidelines, with no statistical difference in performance among different operator groups. The system's cost-effectiveness, automation and performance indicate that it can be successfully translated for use in low-resource settings where central hematology laboratories are not accessible.

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Section: Comparison Between Results By Trained and Untrained Userssupporting

confidence: 79%

Performance of a cost‐effective and automated blood counting system for resource‐limited settings operated by trained and untrained users

Xie

Liu

Tong

et al. 2017

Journal of Biophotonics

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show abstract

“…In addition to RBC lysis, fluorescent labeling of a clinical blood sample is also required. [6,7] Typically, fluorescence staining is performed by applying a cocktail of fluorophore-labeled antibodies to detect specific types of leukocytes. The main limitations include the susceptibility of organic fluorophores to photobleaching which might lead to false results, while the use of expensive antibody reagents that lack long-term stability also add significant cost to Complete blood count with leukocyte (white blood cell, WBC) differential is one of the most frequently ordered clinical test for disease diagnosis.…”

Section: Doi: 101002/smll201903328mentioning

confidence: 99%

“…To overcome this major challenge, a lysis‐free protocol for whole blood sample preparation is highly desired to enable faster and more reliable blood analysis. In addition to RBC lysis, fluorescent labeling of a clinical blood sample is also required . Typically, fluorescence staining is performed by applying a cocktail of fluorophore‐labeled antibodies to detect specific types of leukocytes.…”

Section: Introductionmentioning

confidence: 99%

“…Typically, fluorescence staining is performed by applying a cocktail of fluorophore‐labeled antibodies to detect specific types of leukocytes. The main limitations include the susceptibility of organic fluorophores to photobleaching which might lead to false results, while the use of expensive antibody reagents that lack long‐term stability also add significant cost to the diagnostic test . Thus, it remains a challenging and urgent need for developing multifunctional fluorescent reagents capable of lysis‐free counting and/or differentiating WBCs in whole blood directly toward faster, cheaper, and more reliable CBC for disease diagnostics.…”

Section: Introductionmentioning

confidence: 99%

“…[1,2] There are three major types the diagnostic test. [7] Thus, it remains a challenging and urgent need for developing multifunctional fluorescent reagents capable of lysis-free counting and/or differentiating WBCs in whole blood directly toward faster, cheaper, and more reliable CBC for disease diagnostics.…”

Section: Introductionmentioning

confidence: 99%

See 2 more Smart Citations

Development of Blood‐Cell‐Selective Fluorescent Biodots for Lysis‐Free Leukocyte Imaging and Differential Counting in Whole Blood

Zheng

Tan

2019

Small

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Complete blood count with leukocyte (white blood cell, WBC) differential is one of the most frequently ordered clinical test for disease diagnosis. Herein, multifunctional fluorescent carbon dots derived from biomolecules (biodots) for rapid lysis‐free whole blood analysis are developed. Specifically, two types of biodots are molecularly engineered through hydrothermal synthesis for differential blood cells labeling. Type I biodots synthesized from amino acid (serine/threonine) precursors and passivated with polyethylenimine can label both red blood cells (RBCs) and WBCs with excellent contrast in fluorescence intensity, enabling direct counting of leukocytes in whole blood samples without a tedious RBC lysis step. It also allows three‐part leukocyte differential counting by flow cytometry without using expensive fluorophore‐conjugated antibodies. On the other hand, Type II biodots synthesized from the same amino acid precursors but passivated with a biopolymer (chitosan) are able to selectively lyse RBCs with greater than 98% efficiency to allow simultaneous fluorescent labeling of leukocytes for WBC counting in whole blood. It is envisioned that these novel nanoreagents, which eliminate the cumbersome lysis and antibody conjugation steps for selective labeling of different blood cells, would revolutionize disease diagnostics toward achieving faster, cheaper, and more accurate whole blood analyses in one test.

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A microfluidic cytometer for white blood cell analysis

Peng

Cheng

et al. 2021

Cytometry Pt A

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Despite the wide use of cytometry for white blood cell classification, the performance of traditional cytometers in point-of-care testing remains to be improved.Microfluidic techniques have been shown with considerable potentials in the development of portable devices. Here we present a prototype of microfluidic cytometer which integrates a three-dimensional hydrodynamic focusing system and an on-chip optical system to count and classify white blood cells. By adjusting the flow speed of sheath flow and sample flow, the blood cells can be horizontally and vertically focused in the center of microchannel. Optical fibers and on-chip microlens are embedded for the excitation and detection of single-cell. The microfluidic chip was validated by classifying white blood cells from clinical blood samples.

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Considerations for point-of-care diagnostics: evaluation of acridine orange staining and postprocessing methods for a three-part leukocyte differential test

Cited by 17 publications

References 34 publications

Performance of a cost‐effective and automated blood counting system for resource‐limited settings operated by trained and untrained users

Performance of a cost‐effective and automated blood counting system for resource‐limited settings operated by trained and untrained users

Development of Blood‐Cell‐Selective Fluorescent Biodots for Lysis‐Free Leukocyte Imaging and Differential Counting in Whole Blood

A microfluidic cytometer for white blood cell analysis

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